PORCINE PROPARATHYROID HORMONE
Porcine Proparathyroid Hormone. Identification, Biosynthesis, and Partial Amino Acid Sequence? Luke L. H. Chu, Wei-Yong Huang, E. Travis Littledike,$ James W. Hamilton. and David V. Cohn*
ABSTRACT:
Porcine parathyroid gland slices were incubated with 3H-labeled amino acids in order to label tissue proteins. After incubation a crude hormonal extract was prepared and analyzed by chromatography on carboxymethylcellulose. Among the three radioactive peaks which were detected in the eluate, two were identified as parathyroid hormone and proparathyroid hormone. Based on thin layer gel filtration in the presence of 6 M guanidine-HC1, the proparathyroid hormone had a molecular weight of 11,500 compared to about 9600 for parathyroid hormone. Radioisotope sequence analysis of the proparathyroid hormone
revealed a partial sequence o f Lysl-Pro2-Ile3-Lys4-LysSArg6-Ser7-Val8-Ser9--Ile1 '--Met 14--Gly18--Ser22-Ser23---. Thus, from position 7 onward the relative position of each amino acid tested in this molecule corresponded exactly to that in the porcine parathyroid hormone sequence. The conservation of a similar, though not identical, basic hexapeptide grouping Lys-X-Y-Lys-Lys-Arg- at the amino terminal region of the prohormone in all species examined thus far (porcine, human, and bovine) suggests that this segment of the molecule may play an important role in the conversion of the prohormone to the hormone.
E o p a r a t h yroid hormone (ProPTH) has been discovered to be the biosynthetic precursor of parathyroid hormone in bovine (Hamilton et ai., 1971a; Cohn et aI., 1972; Kemper et al., 1972), human (Habener et al., 1972; Chu et al., 1973a), rat (Chu et al., 1973b), and chicken (MacGregor et al., 1973) parathyroid glands. In all of these species, the prohormone appears to consist of a single peptide chain. The partial amino acid sequences of the amino-terminal region of the bovine and human prohormones have been reported recently (Hamilton et al., 1974; Jacobs et al., 1974; Huang et al., 1975). Both molecules start at the amino-terminus with the identical hexapeptide sequence Lys-Ser-ValLys-Lys-Arg- which is followed by the sequence of the respective PTH molecule. Evidence exists also that the b- and hProPTH's both contain an additional peptide subsequent to the carboxy-terminus of the hormone sequence (Huang et al., 1975; Hamilton et al., 1975). It is visualized that conversion of ProPTH to PTH entails specific cleavages of these amino- and carboxy-terminal peptides (Hamilton et al., 1975). Recently the complete amino acid sequence for porcine PTH was reported (Sauer et al., 1974). Since ProPTH has been found in the parathyroid glands of all animal species examined thus far, it seemed likely that pProPTH would
also exist. If ProPTH exists, one might naturally ask whether its general structure relative to PTH is the same as those two already described. More specifically, does it contain the same amino-terminal hexapeptide as do b- and hProPTH? Answers to these questions should be of aid to our understanding of the mechanisms of the biological conversion of ProPTH to PTH. For this reason, we initiated a study on the biosynthesis of PTH in the porcine parathyroid gland. This report describes the identification and biosynthesis of both ProPTH and PTH by porcine parathyroid gland slices; provides data on the partial amino acid sequence of the porcine prohormone; and compares the porcine prohormone to its bovine and human counterparts.
t From the Calcium Research Laboratory, Veterans Administration Hospital, Kansas City, Missouri 641 28, the University of MissouriKansas City School of Dentistry, Kansas City, Missouri 64108, and the University of Kansas School of Medicine, Kansas City, Kansas 66103. Received February 3, 1975. This work was supported in part by National Institutes of Health Grant AM 15951 from the National Institute of Arthritis, Metabolism and Digestive Diseases. Present address: National Animal Disease Center, USDA, ARS, Ames, Iowa 50010. * To whom correspondence should be addressed at the Calcium Research Laboratory, Veterans Administration Hospital. Abbreviations used are: PTH, parathyroid hormone; ProPTH, proparathyroid hormone; b-, h-, and p- preceding PTH or ProPTH refer to the bovine, human, and porcine molecules, respectively; I-PTH, immunoreactive PTH; C13CCOOH powder, trichloroacetic acid powder (a crude hormonal preparation from parathyroid glands); CM-cellulose, carboxymethylcellulose.
*
Experimental Section Methods Isolation of Radioactive Peptides. Incubation of fresh porcine parathyroid glands with 3H-labeled amino acid was performed as described earlier for human parathyroid gland (Chu et al., 1973a). In some studies which were designed to determine the amino acid sequence of pProPTH and pPTH, combinations of two amino acids-one 3H-labeled and one 14C-labeled-were used instead of a single 3H-labeled amino acid. After incubation, the mixture was frozen quickly until it was processed. To each thawed sample of incubated porcine parathyroid tissue and incubation medium was added 3 g of nonradioactive bovine or porcine parathyroid tissue and the mixture was processed as described earlier for the isolation of the rat and human PTH and ProPTH (Chu et al., 1973a,b). In this procedure the tissue is homogenized in the urea-HCI-cysteine solution and subjected to organic solvent, salt, and trichloroacetic acid precipitation to yield a Cl3CCOOH powder. This is then subjected to ion-exchange chromatography on carboxymethylcellulose in order to separate ProPTH and PTH from each other and from other labeled proteins. Migration Behavior of pProPTH and pPTH on Sephadex Gels. Thin layer gel filtration (Sephadex G-100, superBIOCHEMISTRY, VOL.
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FRACTION FIGURE 1 : CM-cellulose chromatography of porcine parathyroid C13CCOOH powder. The C13CCOOH powder was prepared from a mixture of 40 mg of porcine parathyroid tissue which was incubated for 2 hr and 3 g of carrier porcine tissue. The sample was applied to a CM-cellulose column (2.5 X 100 mm) and eluted with a linear ammonium acetate gradient from 0.01 M , pH 5.3 to 0.30 M , pH 7.0 containing 1 m M mercaptoethanol. Fractions of 1 .5 ml were collected.
tory (Hamilton et al., 1971b) was used to construct the standard curve. The porcine C13CCOOH powder yielded an assay curve which was superimposable on the curve obtained with bPTH standard.
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